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一种适用于监测癌症临床试验样本中CD8 +和CD4 + T细胞反应的强大的人类T细胞培养方法。

A robust human T-cell culture method suitable for monitoring CD8+ and CD4+ T-cell responses from cancer clinical trial samples.

作者信息

Jackson Heather M, Dimopoulos Nektaria, Chen Qiyuan, Luke Tina, Yee Tai Tsin, Maraskovsky Eugene, Old Lloyd J, Davis Ian D, Cebon Jonathan, Chen Weisan

机构信息

Ludwig Institute for Cancer Research, Melbourne Branch, Austin Health, Heidelberg VIC 3084, Australia.

出版信息

J Immunol Methods. 2004 Aug;291(1-2):51-62. doi: 10.1016/j.jim.2004.04.017.

Abstract

Many tumor antigenic determinants have been identified and included in cancer clinical trials. Due to low T-cell frequencies even after vaccination, few T-cell responses can be revealed ex vivo without in vitro stimulation. Various expansion protocols have been employed for this purpose and the outcomes tend to be quite variable, partly due to the high complexity involved in the protocols. Here we systematically studied various common culture conditions including sera, cytokines and feeders and describe a reliable "bulk" culture method that is robust, simpler and more economical. We demonstrated that fetal calf serum (FCS) supported T-cell proliferation better than multiple commercially available pooled human AB sera. IL-2 is critical in our cultures, but IL-7, IL-15 and anti-CTLA-4 in combination with IL-2 did not further enhance T-cell expansion. We typically achieve more than a 40-fold expansion within a 10-day culture period for antigen-specific T cells measured by HLA-peptide tetramer before and after culture. This method was not only validated by multiple operators as a standard operating procedure for monitoring T-cell responses but was also successfully used for discovering novel CD8+ and CD4+ T cells specific to previously unknown epitopes from the NY-ESO-1 tumor antigen.

摘要

许多肿瘤抗原决定簇已被识别并纳入癌症临床试验。由于即使在接种疫苗后T细胞频率仍较低,若不进行体外刺激,几乎无法在体外检测到T细胞反应。为此人们采用了各种扩增方案,但其结果往往差异很大,部分原因是这些方案涉及的复杂性较高。在此,我们系统地研究了包括血清、细胞因子和饲养细胞在内的各种常见培养条件,并描述了一种可靠的“批量”培养方法,该方法稳健、更简单且更经济。我们证明,胎牛血清(FCS)比多种市售混合人AB血清更能支持T细胞增殖。IL-2在我们的培养中至关重要,但IL-7、IL-15以及抗CTLA-4与IL-2联合使用并未进一步增强T细胞扩增。在培养前后,通过HLA-肽四聚体检测,我们通常能在10天的培养期内使抗原特异性T细胞扩增超过40倍。该方法不仅被多个操作人员验证为监测T细胞反应的标准操作程序,还成功用于发现针对NY-ESO-1肿瘤抗原中先前未知表位的新型CD8+和CD4+ T细胞。

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